Light Reflected from Colored Mulches to Growing Turnip Leaves Affects Glucosinolate and Sugar Contents of Edible Roots

Abstract— Plastic mulches are widely used to conserve water and control weeds with less applied herbicides in production of food crops. Both yield and quality are important and can be affected by reflected blue (B), red (R) and far-red (FR) light combinations received during growth and development. Photosynthate allocation among growing plant parts and flavor of edible roots were studied in turnip ( Brassica rapa L.) grown in trickle-irrigated field plots with blue, green and white mulches. The blue and green mulches reflected different amounts of B, but they both reflected FR/R ratios higher than the ratio in incoming sunlight. The white mulch reflected more photosyn-thetic light and a lower FR/R ratio than the blue or green mulches. Plants grown with blue and green mulches did not differ significantly in leaf length, root size and shoot/ root biomass ratio. Those grown with white had shorter leaves and larger roots. Taste testers found that plants grown with blue mulch developed roots with a sharp flavor, and roots from plants grown with green mulch had a mild flavor. Those grown with white had a less distinct flavor. Roots grown with blue mulch had the greatest concentrations of total glucosinolates (GSL) and ascorbic acid. Reducing sugar concentrations were higher in roots grown with green than in those grown with blue mulches. The comparison of chemical composition of roots from plants grown with blue versus green mulches is important because the main difference was the amount of reflected B, suggesting that B influenced an enzyme involved in the pathway from glucose to GSL. We conclude that the spectrum of light reflected from mulch on the soil surface can influence not only shoot/root biomass ratio but also flavor-related chemical composition of field-grown food crop plants.     

Application of fast ultrasound water-bath assisted enzymatic hydrolysis--high performance liquid chromatography-inductively coupled plasma-mass spectrometry procedures for arsenic speciation in seafood materials

Enzymatic hydrolysis of seafood materials for isolating arsenic species (As(III), As(V), DMA and AsB) has been successfully performed by assisting the procedure with ultrasound energy (35 kHz) supplied by an ultrasound water-bath. The use of pepsin, as a proteolytic enzyme, under optimized operating conditions (pH 3.0, temperature 40 °C, enzyme to sample ratio of 0.3) led to an efficient assistance of the enzymatic process in a short period of time (from 4.0 to 30 min). The enzymatic extract was then subjected to a clean-up procedure based on ENVI-Carb™ solid phase extraction (SPE). An optimized anion exchange high performance liquid chromatography (HPLC) coupled to inductively coupled plasma-mass spectrometry (ICP-MS) permitted the fast separation (less than 15 min) of six different arsenic species (arsenite, As(III); arsenate, As(V); dimethylarsinic acid, DMA; and arsenobetaine, AsB; as well as monomethylarsonic acid, MMA; and arsenocholine, AsC) in a single run. Relative standard deviations (n = 11) of the over-all procedure were 7% for AsB and DMA, 11% for As(III) and 9% for MMA. HPLC–ICP-MS determinations were performed using aqueous calibrations covering arsenic concentrations of 0, 5, 10, 25, 100 and 200 μg L⁻¹ (expressed as arsenic) for As(III), As(V), MMA, DMA and AsC; and 0, 125, 250, 500, 750, 1000 and 2000 μg L⁻¹ (expressed as arsenic) for AsB. Germanium (5 μg L⁻¹) was used as an internal standard. Analytical recoveries from the anion exchange column varied from 96 to 105% (enzymatic digests spiked with low target concentrations), from 97 to 104% (enzymatic digests spiked with intermediate target concentrations), and from 98 to 103% (enzymatic digests spiked with high target concentrations). The developed method was successfully applied to two certified reference materials (CRMs), DORM-2 and BCR 627, which offer certified AsB and DMA contents, and also to different seafood samples (mollusks, white fish and cold water fish). Good agreement between certified and found AsB concentrations was achieved when analyzing both CRMs; and also, between certified and found DMA concentrations in BCR 627. In addition, the sum of the different arsenic species concentrations found in most of the analyzed samples was statistically similar to the assessed total arsenic concentrations after a total sample matrix decomposition treatment.     

Characterization of chemiluminescence from singlet oxygen under laminar flow conditions in a micro-channel and its quenching with beverages

Singlet oxygen was generated by reaction of sodium hypochlorite and hydrogen peroxide in a micro-channel. The two reagent solutions were delivered into the micro-channel by a syringe pump, providing a laminar flow liquid-liquid interface. The chemiluminescence from the singlet oxygen was emitted in the collapse of the interface due to molecular diffusion under laminar flow conditions. The chemiluminescence intensity was observed continuously and stably for each combination of reagents fed into the micro-channel; while, in the normal batch-type reactor the chemiluminescence peaks from singlet oxygen were observed within ca. 5 s. The features of the chemiluminescence emitted under laminar flow conditions were examined by changing the concentrations of sodium hypochlorite and hydrogen peroxide; the concentrations of 2.5 mM sodium hypochlorite and 7.5 mM hydrogen peroxide provided highest chemiluminescence intensities without bubble formation. Also, the effects of beverages, such as green tea, coffee, white wine, red wine, and sake (rice wine), on the chemiluminescence intensity as well as the concentrations of sodium hypochlorite and hydrogen peroxide were examined. The chemiluminescence intensities observed with addition of the beverages to the reagents decreased in the following orders; green tea > coffee > red wine > rice wine > white wine (being added to sodium hypochlorite); coffee > white wine > green tea > red wine > rice wine (being added to hydrogen peroxide). It was found that coffee decreased the chemiluminescence intensity (ca. 33% chemiluminescence decrease) without altering the concentrations of sodium hypochlorite or hydrogen peroxide. The cause of the decrease in chemiluminescence with coffee is discussed.     

Differential pulse cathodic stripping voltammetric speciation of trace level inorganic arsenic compounds in natural water samples

A simple, fast and sensitive speciation method is described for inorganic arsenic in water at the μg/l level, applicable in the laboratory and in the field, based on differential pulse cathodic stripping voltammetry (DPCSV). Only As(III) is deposited on a Hg electrode in the presence of Cu and Se in HCl medium. Determination of total As is performed by reducing As(V) to As(III) using sodium meta-bisulfite/sodium thiosulfate reagent stabilized with ascorbic acid. As(V) is quantified by difference. The detection limit (S/N>3) was 0.5 μg/l with a linear range from 4.5 to 180 μg/l. The relative standard deviation (n=6) was 2.4, 2.5, 4.2% for As(III) and 8.0, 6.8, 9.0% for As(V) at levels of 45, 10, and 5 μg/l, respectively. Analysis of the NIST 1640 natural water standard yielded total arsenic concentration 26.5±3.4 μg/l (n=3) compared to the certified value of 26.7 μg/l. Results obtained on several natural water samples analyzed both in the laboratory and on-site compared well with those obtained by HR ICP-MS, GFAAS and IC-AFS. Ions (phosphate, iron, manganese) commonly found in groundwater containing arsenic were found to have negligible interference.     

Controllable three-component luminescence from a 1,8-naphthalimide/Eu(III) complex: white light emission from a single molecule

A macrocycle-appended naphthalimide derivative and its Eu(III) complex show triple luminescence from isolated naphthalimide (blue), aggregated naphthalimide excimers (green) and Eu centres (red) with the balance being sensitive to the degree of aggregation, allowing white light emission to be obtained from a single molecule.     

An organic white light-emitting fluorophore

The synthesis of new benzo[a]- and [b]xanthene dye frameworks is described. A unique benzo[a]xanthene, seminaphtho[a]fluorone (SNAFR-1), is studied in a variety of media. The optimization of solution parameters and excitation wavelengths allows SNAFR-1 to display red, green, and blue emission bands of approximately equal intensities and also to produce white light. Ratiometric red (anion) and green (neutral) emissions are observed upon varying solution pH. A pH-independent violet-blue emission band is due to the addition of nucleophiles to the benzylic carbon of SNAFR-1.     

Blue light induces arsenate uptake in the protist Thraustochytrium

The effects of light on arsenic accumulation of Thraustochytrium CHN‐1 were investigated. Thraustochytrium CHN‐1, when exposed to blue light from light‐emitting diodes (LEDs), accumulated arsenate added to its growth medium to a much greater extent than Thraustochytrium cells exposed to fluorescent or red light, or when cultured in the dark. Arsenic compounds in Thraustochytrium CHN‐1 were analyzed by high‐performance liquid chromatography, with an inductively coupled plasma mass spectrometer serving as an arsenic‐specific detector. Arsenate, arsenite, monomethylarsonic acid (MMAA), dimethylarsinic acid (DMAA) and arsenosugar were identified. The order of arsenic species in Thraustochytrium CHN‐1 was arsenic(V)> arsenic(III)> MMAA > DMAA at an arsenic concentration of 10 mg dm^?3 in the medium in blue LED light. As it is known that blue light induces the synthesis of certain metabolites in plants and microorganisms, this indicates that the accumulation of arsenic is an active metabolic process. Copyright © 2005 John Wiley & Sons, Ltd.     

Escherichia coli: Dominance of Red Light over Other Visible Light Sources in Establishing Viable but Nonculturable State

In this study, the effect of UV-A and different wavelengths of visible light irradiations combined with or without a photosensitizer (methylene blue, MB) on the establishment of viable but nonculturable (VBNC) state in Escherichia coli was investigated. Survival of the E. coli was investigated by measuring plate counts, respiring cell count (RCC), direct viable count (DVC) and total counts over a period of up to 72 h. The inhibition rates of various light sources in the presence or absence of MB on E. coli in seawater were ranked in the order UV-A>red light>white light>blue light>green light (from greatest to least activation). E. coli survived for 10.2, 19.0, 21.3 and 24.04 h under exposure to red, white, blue and green light and for 6.8 h under exposure to UV-A in the presence of MB according to t ₉₉ . Although the VC declined to undetectable levels in a relatively short time, the RCC showed that some cells were still capable of respiration and, therefore, are assumed to have entered the VBNC phase. This is the first time that red light has been shown to have a stronger effect on E. coli survival and VBNC than white, green and blue light in seawater environment.     

Effect of light quality on the accumulation of photosynthetic pigments, proteins and mycosporine-like amino acids in the red alga Porphyra leucosticta (Bangiales, Rhodophyta)

The effect of different light qualities (white, blue, green, yellow and red light) on photosynthesis, measured as chlorophyll fluorescence, and the accumulation of photosynthetic pigments, proteins and the UV-absorbing mycosporine-like amino acids (MAAs) was studied in the red alga Porphyra leucosticta. Blue light promoted the highest accumulation of nitrogen metabolism derived compounds i.e., MAAs, phycoerythrin and proteins in previously N-starved algae after seven days culture in ammonium enriched medium. Similar results were observed in the culture under white light. In contrast, the lowest photosynthetic capacity i.e., lowest electron transport rate and lowest photosynthetic efficiency as well as the growth rate were found under blue light, while higher values were found in red and white lights. Blue light favored the accumulation of the MAAs porphyra-334, palythine and asterina-330 in P. leucosticta. However, white, green, yellow and red lights favored the accumulation of shinorine. The increase of porphyra-334, palythine and asterina-330 occurred in blue light simultaneous to a decrease in shinorine. The accumulation of MAAs and other nitrogenous compounds in P. leucosticta under blue light could not be attributed to photosynthesis and the action of a non-photosynthetic blue light photoreceptor is suggested. A non-photosynthetic photoreceptor could be also involved in the MAAs interconversion pathways in P. leucosticta.     

A rht-Type Luminescent Zn (II)-MOF Constructed by Triazine Hexacarboxylate Ligand: Tunable Luminescent Performance and White-light Emission Regulation through doping Eu3+/Tb3+

White-light emitting materials have become a hot research field of luminescent MOF (Metal–Organic Framework) because of its high practical application value. Herein, we successfully synthesized and characterized a rht-type fluorescent MOF Zn-TDPAT [H₆TDPAT = 2,4,6-tris(3,5-dicarboxylphenylamino)-1,3,5-triazine] with a topology of (3, 24) connected nodes. A series of MOFs materials x%Tb + y%Eu@Zn-TDPAT were prepared by incorporating different concentrations of green emission center Tb³⁺ and red emission center Eu³⁺ into the blue-emitting Zn-MOF. The luminescence properties of MOFs materials x%Tb + y%Eu@Zn-TDPAT can be effectively adjusted by incorporating different concentrations of Tb³⁺ and Eu³⁺ and can obtain multi-color luminescence properties from blue, blue-green, green, yellow green, yellow, blue-red, yellow-red and white. According to trichromatic mechanism, by reasonably matching the intensity of blue light, green light and red light emitted by x%Tb + y%Eu@Zn-TDPAT at 420, 543 and 616 nm, MOFs materials 0.75%Tb + 5%Eu@Zn-TDPAT, 0.65%Tb + 5.5%Eu@Zn-TDPAT and 0.5%Tb + 7.5%Eu@Zn-TDPAT with white-light emission are obtained. Their CIE coordinates are 0.3162, 0.3345 (0.3162, 0.3345), (0.3138, 0.3339) and (0.3329, 0.3222), respectively, which are very close to ideal white-light emission (0.3333,0.3333).     

Dual-wavelength beta-correction spectrophotometric determination of arsenic in wastewater with ethyl violet

Arsenic has been determined by beta-correction spectrophotometry with ethyl violet (EV) in the presence of sodium nitrite which is an oxidant and effective for removing absorption spectra and increasing analytical sensitivity. Extraction with benzene can separate most other metals ions and concentrate arsenic in wastewater. The beta-correction method can eliminate completely the effect of excess EV in its As colored solution to give the real absorbance of the chelate produced. Sensitivity, precision and accuracy are all increased. Beer's law is obeyed over the range 0-2.0 mg l(-1) at 630 nm and the detection limit of arsenic is 0.02 mg l(-1). The results show that the relative standard deviation was less than 12% with the recovery between 91.0 and 114%.     

Adsorption of As(III) from aqueous solutions by iron oxide-coated sand

Arsenic is a toxic element and may be found in natural waters as well as in industrial waters. Leaching of arsenic from industrial wastewater into groundwater may cause significant contamination, which requires proper treatment before its use as drinking water. The present study describes removal of arsenic(III) on iron oxide-coated sand in batch studies conducted as a function of pH, time, initial arsenic concentration, and adsorbent dosage. The results were compared with those for uncoated sand. The adsorption data fitted well in the Langmuir model at different initial concentration of As(III) at 20 g/l fixed adsorbent dose. Maximum adsorption of As(III) for coated sand is found to be much higher (28.57 microg/g) than that for uncoated sand (5.63 microg/g) at pH 7.5 in 2 h. The maximum As(III) removal efficiency achieved is 99% for coated sand at an adsorbent dose of 20 g/l with initial As(III) concentration of 100 microg/l in batch studies. Column studies have also been carried out with 400 microg/l arsenic (pH 7.5) by varying the contact time, filtration rate, and bed depth. Results of column studies demonstrated that at a filtration rate of 4 ml/min the maximum removal of As(III) observed was 94% for coated sand in a contact time of 2 h. The results observed in batch and column studies indicate that iron oxide-coated sand is a suitable adsorbent for reducing As(III) concentration to the limit (50 microg/l) recommended by Indian Standards for Drinking Water.     

RELATIONSHIP BETWEEN LIGHT QUALITY DEPENDENCE AND IRRADIANCE ADAPTATION OF PHOTOSYNTHESIS IN Acetabularia mediterranea*

Characteristic differences in the light intensity curves of photosynthesis after growth of cells of Acetabularia mediterranea Lamour. (A. acetabulum (L.) Silva) in weak and strong white light were similar to those for red and blue light-treated cells, respectively. This indicated that responses to white light quantity and those to light quality might be causally related. Small differences in the thylakoid polypeptide composition of cells grown in high and low intensities of white light were not significant and thus did not help to clarify whether the adaptations to blue or red light, respectively, were the same. When the red to blue-light ratio was varied, keeping the total photon fluence rate constant, the photosynthetic capacity (red light saturated O₂-production) was dependent on blue light irradiance in a logarithmic fashion. The specific influence of red light was not detectable, indicating that only blue light was effective for light irradiance adaptation in Acetabularia. The situation was different, at least for a transient period, when adaptation to light irradiance was allowed to proceed from a low photosynthetic activity after preirradiation of the cells with prolonged red light. The effect of low white light irradiances was pronounced, causing a maximum increase of photosynthetic activity within 3 days. The response to blue light was enhanced as well, and a very low photon irradiance added to continuous red light caused a change of the same order as that produced by high irradiances of blue light alone. This elevated action of low intensity white and blue light is most likely due to increased metabolite supply derived from the degradation of starch enhanced by this light quality. Therefore, photosynthetic effectiveness in Acetabularia is regulated by the irradiance of blue light and by feedback via photosynthetic products.     

Molecular design of efficient white‐light‐emitting fluorene‐based copolymers by mixing singlet and triplet emission

A new strategy to realize efficient white‐light emission from a binary fluorene‐based copolymer (PF‐Phq) with the fluorene segment as a blue emitter and the iridium complex, 9‐iridium(III)bis(2‐(2‐phenyl‐quinoline‐N,C³′)(11,13‐tetradecanedionate))‐3,6‐carbazole (Phq), as a red emitter has been proposed and demonstrated. The photo‐ and electroluminescence properties of the PF‐Phq copolymers were investigated. White‐light emission with two bands of blue and red was achieved from the binary copolymers. The efficiency increased with increasing concentration of iridium complex, which resulted from its efficient phosphorescence emission and the weak phosphorescent quenching due to its lower triplet energy level than that of polyfluorene. In comparison with the binary copolymer, the efficiency and color purity of the ternary copolymers (PF‐Phq‐BT) were improved by introducing fluorescent green benzothiadiazole (BT) unit into polyfluorene backbone. This was ascribed to the exciton confinement of the benzothiadiazole unit, which allowed efficient singlet energy transfer from fluorene segment to BT unit and avoided the triplet quenching resulted from the higher triplet energy levels of phosphorescent green emitters than that of polyfluorene. The phosphorescence quenching is a key factor in the design of white light‐emitting polyfluorene with triplet emitter. It is shown that using singlet green and triplet red emitters is an efficient approach to reduce and even avoid the phosphorescence quenching in the fluorene‐based copolymers. The strategy to incorporate singlet green emitter to polyfluorene backbone and to attach triplet red species to the side chain is promising for white polymer light‐emitting diodes. © 2007 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem 46: 453–463, 2008     

PHOTOINHIBITION OF GROWTH OF- A YELLOW AND A COLORLESS FORM OF CHLAMYDOMONAS REINHARDTII*

Abstract— Long-term growth on acetate in darkness of a permanently yellow and a white-in-darkness mutant of Chlamydomonus reinhardtii showed no requirement for light. Room light or moderate intensities of white light severely inhibited the white mutant, but allowed continuous growth of the yellow form. Blue light (460 nm) stops motility and growth, and induces clumping, in the white form at energy levels which only reduce the growth rate of the yellow mutant. Green light (550 nm) had no effect on either strain, while red light (630 nm), at equal energy levels, affected the white mutant only, however, not as severely as blue light. The mechanism of action of blue and red light is unknown. Evidence suggested the inhibition is not due to cell exudates.     

Effects of Light‐emitting Diode Radiations on Human Retinal Pigment Epithelial Cells In Vitro

Human visual system is exposed to high levels of natural and artificial lights of different spectra and intensities along lifetime. Light‐emitting diodes (LEDs) are the basic lighting components in screens of PCs, phones and TV sets; hence it is so important to know the implications of LED radiations on the human visual system. The aim of this study was to investigate the effect of LEDs radiations on human retinal pigment epithelial cells (HRPEpiC). They were exposed to three light–darkness (12 h/12 h) cycles, using blue‐468 nm, green‐525 nm, red‐616 nm and white light. Cellular viability of HRPEpiC was evaluated by labeling all nuclei with DAPI; Production of reactive oxygen species (ROS) was determined by H2DCFDA staining; mitochondrial membrane potential was quantified by TMRM staining; DNA damage was determined by H2AX histone activation, and apoptosis was evaluated by caspases‐3,‐7 activation. It is shown that LED radiations decrease 75–99% cellular viability, and increase 66–89% cellular apoptosis. They also increase ROS production and DNA damage. Fluorescence intensity of apoptosis was 3.7% in nonirradiated cells and 88.8%, 86.1%, 83.9% and 65.5% in cells exposed to white, blue, green or red light, respectively. This study indicates three light–darkness (12 h/12 h) cycles of exposure to LED lighting affect in vitro HRPEpiC.     

High red,green, and blue color purity electroluminescence from MEH‐PPV and polyalkyfluorenes‐based bright white polymer light emitting displays

A series of white polymer light emitting displays (PLEDs) based on a polymer blend of polyalkylfluorenes and poly(2‐methoxy‐5,2′‐ethyl‐hexyloxy‐1,4‐phenylene vinylene) (MEH‐PPV) was developed. MEH‐PPV or red light emitting alkyfluorene copolymer (PFR) was blended with blue light emitting alkyfluorene copolymer (PFB), and MEH‐PPV was blended with both green light emitting alkyfluorene copolymer (PFG) and PFB to generate white light emission PLEDs. Low turn on voltage (2.7 V), high brightness (12,149 nits), high efficiency (4.0 cd/A, 4.0 lm/W), and good color purity (Commission Internationale de L'Eclairage (CIE_x,y) co‐ordinates (0.32, 0.34)) were obtained for the white PLEDs based on the PFB and MEH‐PPV polymer blend. Exciplex formation in the interface between PFR and PFB induced a new green emission peak for these two components based white PLEDs. As a result, strong white emission (4078 nits) was obtained by mixing the red, green, and blue (RGB) three primary colors. High color purity of blue (CIE, x = 0.14, y = 0.08), green (CIE, x = 0.32, y = 0.64) and red (CIE, x = 0.67, y = 0.33) emissions was achieved for white PLEDs combining with dielectric interference color‐filters. © 2006 Wiley Periodicals, Inc. J Polym Sci Part B: Polym Phys 45: 330–341, 2007     

Upconversion properties of Er3+, Yb3+ and Tm3+ codoped fluorophosphate glasses

Er3+, Yb3+ and Tm3+ codoped fluorophosphate glasses emitting blue, green and red upconversion luminescence at 970 nm laser diode excitation were studied. It was shown that Tm3+ behaves as the sensitizer to Er3+ for the green upconversion luminescence through the energy transfer process: Tm3+:3H4+Er3+:4I 15/2-->Er3+:4I 9/2+Tm3+:3H6, and for the red upconversion luminescence through the energy transfer process: Tm3+:3F4+Er3+:4I 11/2-->Tm3+:3H6+Er3+:4F 9/2. Moreover, Er3+ acts as quenching center for the blue upconversion luminescence of Tm3+. The sensitization of Tm3+ to Er3+ depends on the concentration of Yb3+. The intensity of blue, green and red emissions can be changed by adjusting the concentrations of the three kinds of rare earth ions. This research may provide useful information for the development of high color and spatial resolution devices and white light simulation.     

Determination of trace arsenic in hydrofluoric acid by hydride generation and atomic absorption spectrometry

Practical procedures are given for determination of arsenic(III) and (V) in hydrofluoric acid by means of hydride generation and atomic absorption spectrometry. Arsenic(III) can be determined by direct generation of arsine with sodium borohydride in hydrochloric/hydrofluoric acid medium, arsenic(V) being only slightly reduced under the conditions used. For its determination, arsenic(V) has to be prereduced with potassium iodide, and even then its reduction to arsenic(III) and then arsine is far from complete. It is possible to determine it in presence of arsenic(III) by a difference method, but this is recommended only if the As(V)/As(III) ratio is greater than 1. Total arsenic can be determined after oxidation of As(III) and evaporation of most of the hydrofluoric acid. The limit of determination is 5 g/l for arsenic(III) and 0.25 g/l for total arsenic; the relative standard deviation is about 10%.